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首页> 外文期刊>Endocrine Research >Application of differential display in the identification of androgen-regulated genes.
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Application of differential display in the identification of androgen-regulated genes.

机译:差异显示在雄激素调节基因鉴定中的应用。

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摘要

Identification of androgen-regulated genes in neurons is an important step in understanding the mechanisms involved in androgen action. The aim of the current study was to identify androgen-responsive genes in the neural cells using the technique of differential display reverse transcription polymerase chain reaction (DDRT-PCR) on the human neuroblastoma cell line, SK-N-MC. Using this analysis, 18 putatively androgen-regulated cDNA species were identified, ranging in size from 280 to 800 bp. Of these, 14 were found to be negatively regulated and 4 positively regulated by androgens. Only 12 were successfully re-amplified, and of these, 8 were found to contain multiple species of cDNA fragments. When Northern analysis was conducted using the 21 different cDNA fragments as probes, only one was found to confirm the androgen regulation demonstrated via DDRT-PCR. While this putatively regulated gene remains to be fully characterized, future studies of may provide insights into the molecular mechanisms governing androgen action in neural cells.
机译:识别神经元中雄激素调节基因是理解雄激素作用机制的重要步骤。本研究的目的是使用人类神经母细胞瘤细胞系SK-N-MC上的差异显示逆转录聚合酶链反应(DDRT-PCR)技术鉴定神经细胞中的雄激素响应基因。使用该分析,鉴定出了18种可能由雄激素调节的cDNA,其大小在280至800 bp之间。其中,有14个受雄激素负调控,有4个受雄激素正调控。仅成功地重新扩增了12个,其中发现8个包含多种cDNA片段。当使用21个不同的cDNA片段作为探针进行Northern分析时,仅发现一个可以确认通过DDRT-PCR证实的雄激素调节。尽管该推定调控的基因仍有待充分表征,但其进一步的研究可能会提供有关控制神经细胞中雄激素作用的分子机制的见解。

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